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Detection of Arthropod-Borne Pathogens Using PCR Techniques

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Detection of Arthropod-Borne Pathogens Using PCR Techniques Melissa Miller Entomologist US Army Center for Health Promotion & Preventive Medicine, – PowerPoint PPT presentation

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Title: Detection of Arthropod-Borne Pathogens Using PCR Techniques


1
Detection of Arthropod-Borne Pathogens Using PCR
Techniques
  • Melissa Miller
  • Entomologist
  • US Army Center for Health Promotion Preventive
    Medicine,
  • Fort George G. Meade, MD

2
Real-Time PCR Protocols
  • Tick-Borne Pathogens
  • Ehrlichia Species
  • E. chaffeensis, E. ewingii, and Anaplasma
    phagocytophilum
  • Hybridization Probes
  • Anaplasma phagocytopilum
  • Hydrolysis Probes
  • Rickettsia
  • Rickettsia spp.
  • Hydrolysis Probes

3
Real-Time PCR Protocols continued
  • Tick-Borne Pathogens
  • Borrelia Species
  • B. burgdorferi
  • Hydrolysis Probes
  • Borrelia spp.
  • Hydrolysis Probes

4
Conventional PCR Protocols
  • Tick-Borne Pathogens
  • Borrelia Species
  • B. burgdorferi OspA
  • Borrelia spp. FLA
  • Ehrlichia Species
  • E. chaffeensis
  • Anaplasma phagocytophilum

5
Conventional PCR Protocols continued
  • Tick-Borne Pathogens
  • Rickettsia
  • Rickettsia spp.
  • RFLP to species

6
DETECTION OF ARTHROPOD-BORNE PATHOGENS USING
REAL-TIME POLYMERASE CHAIN REACTION TECHNIQUES
  • Real-time techniques for detection of DNA from
    tick-borne pathogens
  • Hydrolysis Probes

FRET-Fluorescence Resonance Energy Transfer
Emission FRET
Hybridization
Cleavage
Graphics from the Second Joint Symposium on Food
Safety and Nutrition kindly provided by Dr.Guy
Van den Eede
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DETECTION OF ARTHROPOD-BORNE PATHOGENS USING
REAL-TIME POLYMERASE CHAIN REACTION TECHNIQUES
  • Real-time techniques for detection of DNA from
    tick-borne pathogens
  • Hybridization Probes
  • FRET-Fluorescence Resonance Energy Transfer

Emission FRET
Amplification
Hybridization
Graphics courtesy of Roche Molecular Biochemicals
Inc.
18
Melting Curve Analysis
  • Sequence Confirmation
  • Highly Specific
  • Each product has a specific TM
  • Take advantage of different fluorescent dyes and
    formats
  • Eliminates inclusion of primer-dimers

19
E. ewingii 55.15 º C
A. phagocytophila 68.81 ºC
E. chaffeensis 62.63 º C
20
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